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Journal of Lipid Research, Vol 17, 516-526, Copyright © 1976 by Lipid Research, Inc.
RD Harper and ED Saggerson
Fat cells isolated from rat epididymal adipose tissue were incubated with
albumin-bound [14C]palmitate. Incorporation of 14C into 14CO2 and
glycerides was measured. Some evidence is presented to suggest that the
exogenous palmitate pool is in isotopic equilibrium with intracellular
precursors for these metabolic processes. Precautions were taken to
minimize dilution of the exogenous palmitate pool by fatty acids released
from the cells. 14CO2 production from [1-14C]palmitate was 3 times that
from [16-14C]palmitate. Octanoate increased this differential oxidation of
palmitate carbons and also inhibited palmitate oxidation without similarly
affecting esterification. Glucose increases palmitate esterification in
cells from fed or starved rats. Insulin potentiated this effect of glucose.
Glucose influenced palmitate oxidation in a more complex manner, dependent
upon the glucose concentration. Both the observation that esterification
constitutes 99% of the metabolic flux of fatty acid and the manner in which
glucose, insulin, or starvation influence palmitate esterification and
oxidation suggested that factors controlling esterification may alter
oxidation as a secondary effect, but not vice versa. It is suggested that
oxidation and esterification compete for a single intracellular precursor,
possibly extramitochondrial long chain fatty acyl CoA.
ARTICLES
Factors affecting fatty acid oxidation in fat cells isolated from rat white adipose tissue
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